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Polyacrylamide gels for rapid casting, blotting, and imaging, with storage stability

a technology of polyacrylamide gels and stable storage, applied in the direction of fluid pressure measurement, liquid/fluent solid measurement, peptides, etc., can solve the problems of protein denatured, loss of three-dimensional shape, close molecular weight, etc., to achieve stable for extended lengths of time, little or no deterioration, and the ability to blot

Active Publication Date: 2014-09-18
BIO RAD LAB INC
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Benefits of technology

The patent describes a system and solutions for hand-casting gels, which offer advantages over traditional methods. The gels can be stored for extended periods without deterioration, and the process allows for faster electrophoresis and blotting without using stains. The stock solutions are also more stable than some other stock solutions. Overall, the system provides a more efficient and effective way to handle protein samples.

Problems solved by technology

In the presence of SDS, however, proteins become denatured, i.e., they unfold and thereby lose their characteristic three-dimensional shapes.
Certain proteins are very close in molecular weight, however, which makes them difficult to separate in SDS-PAGE.
Unfortunately, casting a gel is a time-consuming and labor-intensive procedure, and for this reason it has become commonplace for researchers to purchase pre-formed gels rather than to cast a gel at its point of use.
Another difficulty concerns the electric field strength at which a gel is run and the length of time involved in completing a run.
Hand-cast gels are typically run at low field strength to avoid heating the gel during the run, since heating causes artifacts in the experiment, and the lower the field strength the longer the time required to achieve protein separation.
Staining also takes time.
While pre-cast gels have advantages, they also have disadvantages.
One disadvantage is that they are more expensive than hand-cast gels, since the manufacturer will pass on to the user the cost of making, storing, and distributing the gels.
A second disadvantage is that the user is limited to the types of gels that the manufacturers make available.
With hand-cast gels, the user can customize the resolving gel by personally selecting monomer solutions of specific compositions to meet the special needs or interests of a particular experiment, but such flexibility is typically unavailable with precast gels.
Despite its benefits, therefore, hand cast gels typically lack many of the desirable properties of manufactured pre-cast gels, including the ability to store gels for future use, run the gels quickly, visualize proteins without staining procedures, and quickly transfer the protein bands from the gels to membranes and confirm successful protein transfer on membrane without staining

Method used

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Examples

Experimental program
Comparison scheme
Effect test

Embodiment Construction

[0021]I. Hand Cast Gels

[0022]As noted above, handcast gels and systems comprising such gels are provided. Handcast gels as described herein can be continuous (i.e., a gel comprising only a resolving portion) or dis-continuous (i.e., a gel comprising a stacker portion and a resolving portion). In some embodiments, the gels can be stored for a considerable time before use (e.g., more than 7, 14, 21, or 28 days). In some embodiments, the gels are capable of electrophoresis within as short a time as 15 minutes (e.g., measured by the dye front running to the bottom of the gel) and in some embodiments are capable of substantially complete transfer of protein to nitrocellulose or PVDF membrane by blotting in as short a time as 3 minutes in the Bio-Rad Trans-Blot® Turbo™ Transfer System or 15 minutes in a standard tank blot apparatus. In some embodiments, the gels are capable of long storage as noted above, are capable of fast electrophoresis, and fast transfer of proteins during blotting.

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Abstract

Hand cast gels, and solutions for their preparation, are described.

Description

CROSS-REFERENCE TO RELATED PATENT APPLICATIONS[0001]The present application claims benefit of priority to U.S. Provisional Patent Application No. 61 / 793,884, filed Mar. 15, 2013, which is incorporated by reference.BACKGROUND OF THE INVENTION[0002]Polyacrylamide gel electrophoresis (PAGE) is widely used in biotechnology laboratories for the processing of biological samples to separate the biomolecules present in the samples for identification, and in some cases to quantify the separated species. Protein mixtures, peptide mixtures, and mixtures of DNA, RNA, and fragments of DNA and RNA can all be separated on polyacrylamide gels. For protein mixtures, a particularly useful form of PAGE is SDS-PAGE where the detergent sodium dodecyl sulfate (SDS) is included in the sample. All proteins consist of linked amino acid residues and each protein folds naturally into a three-dimensional shape that is characteristic of, and distinctive for, each individual protein. Thus, both the amino acid se...

Claims

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Application Information

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Patent Type & Authority Applications(United States)
IPC IPC(8): G01N27/447B65D85/00
CPCB65D85/70G01N27/44747B01D57/02C07K1/26C08F2/46C08K3/00G01N21/6428
Inventor LI, LEIYANG, XUEMEIBELISLE, CHRISTOPHER
Owner BIO RAD LAB INC
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